CN103181323A - Culture method for blueberry embryoids - Google Patents
Culture method for blueberry embryoids Download PDFInfo
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- CN103181323A CN103181323A CN2011104505317A CN201110450531A CN103181323A CN 103181323 A CN103181323 A CN 103181323A CN 2011104505317 A CN2011104505317 A CN 2011104505317A CN 201110450531 A CN201110450531 A CN 201110450531A CN 103181323 A CN103181323 A CN 103181323A
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Abstract
The invention discloses a culture method for blueberry embryoids. The culture method comprises the steps of preparing a culture medium by using blueberry with 2-3 months old leaves as an explant, preparing a culture medium, sterilizing the explant and inoculating, subculturing calluses, inducing single cells, differentiating the single cells and culturing the embryoids. The calluses of the blueberry are obtained by induction of the blueberry leaves, the calluses are cultured to obtain the single cells, the single cells are induced to the blueberry embryoids, and the blueberry embryoids are used for culturing the blueberry plants, so that the formation of adventitious buds and vitrified shoots can be reduced and the number of effective seedlings. The calluses can be prevented from browning by using PVP, which is very suitable for the calluses of the blueberry. A culture speed is fast, one hundred thousand of blueberry tissue cultured seedlings can be cultured within five months, and the cultured seedlings have similar growing states basically, high plant qualities and relatively small plant viruses.
Description
Technical field
The present invention relates to a kind of rare fruit kind blueberry embryoid and cultivate, belong to the Plant Tissue Breeding field.
Background technology
Utilize blade to come evoked callus to learn very common in the group training.Blueberry all uses the simple bud branch to organize the differentiation bud of growing thickly, though grow thickly bud than being easier to cultivation, this is very slowly for a large amount of cultivation blueberry nursery stocks.It is that the simple bud branch of tender leaf is cultivated the blueberry plant that the 5th phase in 2007 " Molecular Plant Breeding " Ning Zhi resentment waits with grow thickly inducing of bud and plant regeneration of blueberry, when the excessive concentration of ZT, surpass 2.0 mg/L, can form a large amount of indefinite buds, some callus and vitrifying seedling occur, reduce the quantity of effective seedling; The 9th phase in 2010 " northern gardening ", newly cultivate the blueberry plant in high-amplitude wave etc. slightly with blueberry half materialization, be easy to take place brownization.
Summary of the invention
The technical problem to be solved in the present invention provides a kind of method of fast culture blueberry embryoid.
Technical scheme of the present invention is: a kind of blueberry embryoid cultural method, and as explant, behind the preparation medium, with explant sterilization and inoculation, the callus subculture is induced unicellularly with the blueberry that grows 2-3 month leaf, and embryoid is cultivated in unicellular differentiation.
The prescription of described preparation medium is:
Callus subculture medium prescription: WPM+ZT0.1 ~ 0.5mg/L+2,4-D 1 ~ 4mg/L+NAA 0.3 ~ 1.4mg/L+6-BA 1.0 ~ 4.0mg/L+sucrose 20g/L+PVP 0.5 ~ 1g/L+agar 5.2g/L, PH 5.2 ~ 5.8,25 ℃ of temperature, dark culturing;
Unicellular cultivation prescription: WPM+ZT0.1 ~ 0.5mg/L+2,4-D 1 ~ 4mg/L+NAA0.5 ~ 1.5mg/L+6-BA 1.0 ~ 4.0mg/L+ sucrose 20g/L+PVP 0.5 ~ 1g/L+agar 5.2g/L, PH 5.2 ~ 5.8,25 ℃ of temperature, dark culturing;
Unicellular dedifferentiation prescription: 1/2WPM+6-BA 1.0 ~ 3.0mg/L+NAA0.5 ~ 1.6 mg/L+KT 0.1 ~ 1.5 mg/L+sucrose 15 ~ 40g/L+PVP 0.5g ~ 1 g/L, PH 5.2-5.8,25 ℃ of temperature, dark culturing;
Embryoid is cultivated prescription: WPM+ZT 0.1 ~ 2mg/L+IBA 1.0 ~ 2.0 mg/L+ agar 5.2g/L, and PH 5.2-5.8,25 ℃ of temperature, illumination 12h cultivates.
Described concrete operations with explant sterilization and inoculation are: explant washes 0.5h with flowing water, and explant is cleaned down, and adds several of tweens, is placed under the flowing water and washes 20 ~ 30min; The explant of handling well is with the alcohol 1min that sterilizes, and with the mercuric chloride 3min that sterilizes, with aseptic washing 5 ~ 8 times, puts into sterile water and waits to inoculate again; The explant that sterilization is good cuts the edge with scissors, cuts off vein; Abaxial side upwards is inoculated on the evoked callus medium.
The concrete operations of described callus subculture are: the callus that induces is cut, be inoculated on the callus medium subculture and cultivate, the callus that subculture is grown is twice of subculture again.
Describedly induce single celled concrete operations to be: the callus that subculture is good is inoculated on the subculture liquid nutrient medium, adds perlite, cultivates with 200 rev/mins of concussions.
The concrete operations of described unicellular differentiation are: take out unicellular culture fluid from shaking table, leave standstill, get supernatant liquor, insert the unicellular liquid nutrient medium of inducing then, be placed on that temperature is set as on the shaking table: 25 ℃, revolution 200 commentaries on classics/min cultivated three days night.
The concrete operations of described embryoid cultivation are: muddiness occurs in the bottle behind the concussion cultivation 2-3d, light intensity is adjusted to 5000 luxs, leaves standstill to cultivate 12h again, gets supernatant liquor then and is inoculated on the unicellular inducing culture, cultivation 5-8d.
The invention has the beneficial effects as follows: utilize the blueberry leaf to be induced to the callus of blueberry, again callus is turned out unicellular, again with the unicellular blueberry embryoid that induces, utilize the embryoid of blueberry to cultivate the blueberry plant, reduce the formation of indefinite bud and vitrifying seedling, improve the quantity of effective seedling; Employing PVP just can be so that brownization do not take place in callus, and this is very suitable to the blueberry callus.Cultivation speed is fast, can turn out 100,000 blueberry group training seedlings in five months; . the nursery stock growing way that cultivation is come out is the same substantially; The nursery stock plant quality of turning out is higher, and plant virus is fewer.
Embodiment
Embodiment 1
A kind of blueberry embryoid cultural method is material with being grown in Changbai Mountain, northeast wild blueberry, with growing 2-3 month leaf as explant, behind the preparation medium, with explant sterilization and inoculation, the callus subculture, induce unicellularly, embryoid is cultivated in unicellular differentiation.The prescription of described preparation medium is: callus subculture medium prescription: WPM+ZT0.1mg/L+2,4-D 1mg/L+NAA 0.3mg/L+6-BA 1.0mg/L+sucrose 20g/L+PVP 0.5g/L+agar 5.2g/L, PH 5.2,25 ℃ of temperature, dark culturing; Unicellular cultivation prescription: WPM+ZT0.1mg/L+2,4-D 1mg/L+NAA0.5mg/L+6-BA 1.0mg/L+ sucrose 20g/L+PVP 0.5g/L+agar 5.2g/L, PH 5.2,25 ℃ of temperature, dark culturing; Unicellular dedifferentiation prescription: 1/2WPM+6-BA 1.0mg/L+NAA0.5 mg/L+KT 0.1 mg/L+sucrose 15g/L+PVP 0.5g g/L, PH 5.2,25 ℃ of temperature, dark culturing; Embryoid is cultivated prescription: WPM+ZT 0.1mg/L+IBA 1.0 mg/L+ agar 5.2g/L, and PH 5.2,25 ℃ of temperature, illumination 12h cultivates.With the concrete operations of explant sterilization and inoculation be: explant washes 0.5h with flowing water, and explant is cleaned down, and adds several of tweens, is placed under the flowing water and washes 20 ~ 30min; The explant of handling well is with the alcohol 1min that sterilizes, and with the mercuric chloride 3min that sterilizes, with aseptic washing 5 ~ 8 times, puts into sterile water and waits to inoculate again; The explant that sterilization is good cuts the edge with scissors, cuts off vein; Abaxial side upwards is inoculated on the evoked callus medium.The concrete operations of callus subculture are: the callus that induces is cut, be inoculated on the callus medium subculture and cultivate, the callus that subculture is grown is twice of subculture again.The callus that has just induced is yellow for green band point, and that twice back of subculture callus becomes is faint yellow, and callus is more loose.In the callus subculture is cultivated, can not surpass five times, unicellularly after surpassing five times can not be divided into embryoid.Induce single celled concrete operations to be: the callus that subculture is good is inoculated on the subculture liquid nutrient medium, adds perlite, cultivates with 200 rev/mins of concussions.Adding perlite, be that callus is broken into big cell mass, and big cell mass is being cleaved into small cell cluster, and then is broken into unicellular.The concrete operations of described unicellular differentiation are: take out unicellular culture fluid from shaking table, leave standstill, get supernatant liquor, insert the unicellular liquid nutrient medium of inducing then, be placed on that temperature is set as on the shaking table: 25 ℃, revolution 200 commentaries on classics/min cultivated three days night.The concrete operations of embryoid cultivation are: muddiness occurs in the bottle behind the concussion cultivation 2-3d, light intensity is adjusted to 5000 luxs, leaves standstill to cultivate 12h again, gets supernatant liquor then and is inoculated on the unicellular inducing culture, cultivation 5-8d.A lot of thickly dotted green points again on the solid culture medium, embryoid has begun to sprout, and cultivates the 5-8d media surface and grows leaf and be accompanied by and the root base occurs, after three days, can see bud and the Bai Gen of plant clearly, and embryoid is cultivated success.
Embodiment 2
A kind of blueberry embryoid cultural method is material with being grown in Changbai Mountain, northeast wild blueberry, with growing 2-3 month leaf as explant, behind the preparation medium, with explant sterilization and inoculation, the callus subculture, induce unicellularly, embryoid is cultivated in unicellular differentiation.The prescription of described preparation medium is: callus subculture medium prescription: WPM+ZT0.5mg/L+2,4-D 4mg/L+NAA 1.4mg/L+6-BA 4.0mg/L+sucrose 20g/L+PVP 1g/L+agar 5.2g/L, PH 5.8,25 ℃ of temperature, dark culturing; Unicellular cultivation prescription: WPM+ZT0.5mg/L+2,4-D 4mg/L+NAA1.5mg/L+6-BA 4.0mg/L+ sucrose 20g/L+PVP 1g/L+agar 5.2g/L, PH 5.8,25 ℃ of temperature, dark culturing; Unicellular dedifferentiation prescription: 1/2WPM+6-BA 3.0mg/L+NAA1.6 mg/L+KT 1.5 mg/L+sucrose 40g/L+PVP 1 g/L, PH 5.8,25 ℃ of temperature, dark culturing; Embryoid is cultivated prescription: WPM+ZT 0.1 ~ 2mg/L+IBA 2.0 mg/L+ agar 5.2g/L, and PH 5.8,25 ℃ of temperature, illumination 12h cultivates.With the concrete operations of explant sterilization and inoculation be: explant washes 0.5h with flowing water, and explant is cleaned down, and adds several of tweens, is placed under the flowing water and washes 30min; The explant of handling well is with the alcohol 1min that sterilizes, and with the mercuric chloride 3min that sterilizes, with aseptic washing 8 times, puts into sterile water and waits to inoculate again; The explant that sterilization is good cuts the edge with scissors, cuts off vein; Abaxial side upwards is inoculated on the evoked callus medium.The concrete operations of callus subculture are: the callus that induces is cut, be inoculated on the callus medium subculture and cultivate, the callus that subculture is grown is twice of subculture again.The callus that has just induced is yellow for green band point, and that twice back of subculture callus becomes is faint yellow, and callus is more loose.In the callus subculture is cultivated, can not surpass five times, unicellularly after surpassing five times can not be divided into embryoid.Induce single celled concrete operations to be: the callus that subculture is good is inoculated on the subculture liquid nutrient medium, adds perlite, cultivates with 200 rev/mins of concussions.Adding perlite, be that callus is broken into big cell mass, and big cell mass is being cleaved into small cell cluster, and then is broken into unicellular.The concrete operations of described unicellular differentiation are: take out unicellular culture fluid from shaking table, leave standstill, get supernatant liquor, insert the unicellular liquid nutrient medium of inducing then, be placed on that temperature is set as on the shaking table: 25 ℃, revolution 200 commentaries on classics/min cultivated three days night.The concrete operations of embryoid cultivation are: muddiness occurs in the bottle behind the concussion cultivation 2-3d, light intensity is adjusted to 5000 luxs, leaves standstill to cultivate 12h again, gets supernatant liquor then and is inoculated on the unicellular inducing culture, cultivation 5-8d.A lot of thickly dotted green points again on the solid culture medium, embryoid has begun to sprout, and cultivates the 5-8d media surface and grows leaf and be accompanied by and the root base occurs, after three days, can see bud and the Bai Gen of plant clearly, and embryoid is cultivated success.
Embodiment 3
A kind of blueberry embryoid cultural method is material with being grown in Changbai Mountain, northeast wild blueberry, with growing 2-3 month leaf as explant, behind the preparation medium, with explant sterilization and inoculation, the callus subculture, induce unicellularly, embryoid is cultivated in unicellular differentiation.The prescription of described preparation medium is: callus subculture medium prescription: WPM+ZT0.1 ~ 0.5mg/L+2,4-D 1 ~ 4mg/L+NAA 0.3 ~ 1.4mg/L+6-BA 1.0 ~ 4.0mg/L+sucrose 20g/L+PVP 0.5 ~ 1g/L+agar 5.2g/L, PH 5.2 ~ 5.8,25 ℃ of temperature, dark culturing; Unicellular cultivation prescription: WPM+ZT0.1 ~ 0.5mg/L+2,4-D 1 ~ 4mg/L+NAA0.5 ~ 1.5mg/L+6-BA 1.0 ~ 4.0mg/L+ sucrose 20g/L+PVP 0.5 ~ 1g/L+agar 5.2g/L, PH 5.2 ~ 5.8,25 ℃ of temperature, dark culturing; Unicellular dedifferentiation prescription: 1/2WPM+6-BA 1.0 ~ 3.0mg/L+NAA0.5 ~ 1.6 mg/L+KT 0.1 ~ 1.5 mg/L+sucrose 15 ~ 40g/L+PVP 0.5g ~ 1 g/L, PH 5.2-5.8,25 ℃ of temperature, dark culturing; Embryoid is cultivated prescription: WPM+ZT 0.1 ~ 2mg/L+IBA 1.0 ~ 2.0 mg/L+ agar 5.2g/L, and PH 5.2-5.8,25 ℃ of temperature, illumination 12h cultivates.With the concrete operations of explant sterilization and inoculation be: explant washes 0.5h with flowing water, and explant is cleaned down, and adds several of tweens, is placed under the flowing water and washes 20 ~ 30min; The explant of handling well is with the alcohol 1min that sterilizes, and with the mercuric chloride 3min that sterilizes, with aseptic washing 5 ~ 8 times, puts into sterile water and waits to inoculate again; The explant that sterilization is good cuts the edge with scissors, cuts off vein; Abaxial side upwards is inoculated on the evoked callus medium.The concrete operations of callus subculture are: the callus that induces is cut, be inoculated on the callus medium subculture and cultivate, the callus that subculture is grown is twice of subculture again.The callus that has just induced is yellow for green band point, and that twice back of subculture callus becomes is faint yellow, and callus is more loose.In the callus subculture is cultivated, can not surpass five times, unicellularly after surpassing five times can not be divided into embryoid.Induce single celled concrete operations to be: the callus that subculture is good is inoculated on the subculture liquid nutrient medium, adds perlite, cultivates with 200 rev/mins of concussions.Adding perlite, be that callus is broken into big cell mass, and big cell mass is being cleaved into small cell cluster, and then is broken into unicellular.The concrete operations of described unicellular differentiation are: take out unicellular culture fluid from shaking table, leave standstill, get supernatant liquor, insert the unicellular liquid nutrient medium of inducing then, be placed on that temperature is set as on the shaking table: 25 ℃, revolution 200 commentaries on classics/min cultivated three days night.The concrete operations of embryoid cultivation are: muddiness occurs in the bottle behind the concussion cultivation 2-3d, light intensity is adjusted to 5000 luxs, leaves standstill to cultivate 12h again, gets supernatant liquor then and is inoculated on the unicellular inducing culture, cultivation 5-8d.A lot of thickly dotted green points again on the solid culture medium, embryoid has begun to sprout, and cultivates the 5-8d media surface and grows leaf and be accompanied by and the root base occurs, after three days, can see bud and the Bai Gen of plant clearly, and embryoid is cultivated success.
Claims (7)
1. blueberry embryoid cultural method is characterized in that: as explant, behind the preparation medium, with explant sterilization and inoculation, the callus subculture is induced unicellularly with the blueberry that grows 2-3 month leaf, and embryoid is cultivated in unicellular differentiation.
2. blueberry embryoid cultural method according to claim 1, it is characterized in that: the prescription of described preparation medium is:
Callus subculture medium prescription: WPM+ZT0.1 ~ 0.5mg/L+2,4-D 1 ~ 4mg/L+NAA 0.3 ~ 1.4mg/L+6-BA 1.0 ~ 4.0mg/L+sucrose 20g/L+PVP 0.5 ~ 1g/L+agar 5.2g/L, PH 5.2 ~ 5.8,25 ℃ of temperature, dark culturing;
Unicellular cultivation prescription: WPM+ZT0.1 ~ 0.5mg/L+2,4-D 1 ~ 4mg/L+NAA0.5 ~ 1.5mg/L+6-BA 1.0 ~ 4.0mg/L+ sucrose 20g/L+PVP 0.5 ~ 1g/L+agar 5.2g/L, PH 5.2 ~ 5.8,25 ℃ of temperature, dark culturing;
Unicellular dedifferentiation prescription: 1/2WPM+6-BA 1.0 ~ 3.0mg/L+NAA0.5 ~ 1.6 mg/L+KT 0.1 ~ 1.5 mg/L+sucrose 15 ~ 40g/L+PVP 0.5g ~ 1 g/L, PH 5.2-5.8,25 ℃ of temperature, dark culturing;
Embryoid is cultivated prescription: WPM+ZT 0.1 ~ 2mg/L+IBA 1.0 ~ 2.0 mg/L+ agar 5.2g/L, and PH 5.2-5.8,25 ℃ of temperature, illumination 12h cultivates.
3. blueberry embryoid cultural method according to claim 1, it is characterized in that: described concrete operations with explant sterilization and inoculation are: explant washes 0.5h with flowing water, explant is cleaned down, add several of tweens, be placed under the flowing water and wash 20 ~ 30min; The explant of handling well is with the alcohol 1min that sterilizes, and with the mercuric chloride 3min that sterilizes, with aseptic washing 5 ~ 8 times, puts into sterile water and waits to inoculate again; The explant that sterilization is good cuts the edge with scissors, cuts off vein; Abaxial side upwards is inoculated on the evoked callus medium.
4. blueberry embryoid cultural method according to claim 1, it is characterized in that: the concrete operations of described callus subculture are: the callus that induces is cut, be inoculated on the callus medium subculture and cultivate, the callus that subculture is grown is twice of subculture again.
5. blueberry embryoid cultural method according to claim 1 is characterized in that: describedly induce single celled concrete operations to be: the callus that subculture is good is inoculated on the subculture liquid nutrient medium, adds perlite, cultivates with 200 rev/mins of concussions.
6. blueberry embryoid cultural method according to claim 1, it is characterized in that: the concrete operations of described unicellular differentiation are: take out unicellular culture fluid from shaking table, leave standstill, get supernatant liquor, insert the unicellular liquid nutrient medium of inducing then, be placed on that temperature is set as on the shaking table: 25 ℃, revolution 200 commentaries on classics/min cultivated three days night.
7. blueberry embryoid cultural method according to claim 1, it is characterized in that: the concrete operations that described embryoid is cultivated are: occur muddy behind the concussion cultivation 2-3d in the bottle, light intensity is adjusted to 5000 luxs, leave standstill again and cultivate 12h, get supernatant liquor then and be inoculated on the unicellular inducing culture, cultivate 5-8d.
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CN103598093A (en) * | 2013-10-31 | 2014-02-26 | 李本明 | Inducing method of blueberry embryoid |
CN105851385A (en) * | 2016-05-03 | 2016-08-17 | 泉州正和堂生物科技有限公司 | Dendrobium nobile monomer germ tea and preparation method thereof |
CN106171989A (en) * | 2016-07-13 | 2016-12-07 | 吉林省普蓝高科技有限公司 | Alleviate culture medium of blueberry tissue culture Seedling brownization and preparation method thereof |
CN106171993A (en) * | 2016-07-15 | 2016-12-07 | 华南农业大学 | A kind of with highly efficient regeneration method that Anthocephalus chinensis blade is outer implant |
CN106305385A (en) * | 2016-08-19 | 2017-01-11 | 江苏艺轩园林景观工程有限公司 | Culture method of blueberry |
CN106613939A (en) * | 2016-09-30 | 2017-05-10 | 温州科技职业学院 | Culture medium for indirect regeneration of high-bush blueberry somatic embryos and culture method |
CN106818379A (en) * | 2017-02-20 | 2017-06-13 | 湖北生态工程职业技术学院 | A kind of blueberry seed propagation seedling method |
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Cited By (9)
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CN103598093A (en) * | 2013-10-31 | 2014-02-26 | 李本明 | Inducing method of blueberry embryoid |
CN103598093B (en) * | 2013-10-31 | 2015-10-21 | 青岛文创科技有限公司 | A kind of abductive approach of blueberry embryoid |
CN105851385A (en) * | 2016-05-03 | 2016-08-17 | 泉州正和堂生物科技有限公司 | Dendrobium nobile monomer germ tea and preparation method thereof |
CN106171989A (en) * | 2016-07-13 | 2016-12-07 | 吉林省普蓝高科技有限公司 | Alleviate culture medium of blueberry tissue culture Seedling brownization and preparation method thereof |
CN106171993A (en) * | 2016-07-15 | 2016-12-07 | 华南农业大学 | A kind of with highly efficient regeneration method that Anthocephalus chinensis blade is outer implant |
CN106171993B (en) * | 2016-07-15 | 2019-01-08 | 华南农业大学 | It is a kind of using a variety of millet wood blade as the highly efficient regeneration method of explant |
CN106305385A (en) * | 2016-08-19 | 2017-01-11 | 江苏艺轩园林景观工程有限公司 | Culture method of blueberry |
CN106613939A (en) * | 2016-09-30 | 2017-05-10 | 温州科技职业学院 | Culture medium for indirect regeneration of high-bush blueberry somatic embryos and culture method |
CN106818379A (en) * | 2017-02-20 | 2017-06-13 | 湖北生态工程职业技术学院 | A kind of blueberry seed propagation seedling method |
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